p53 Regulation of G2 Checkpoint Is Retinoblastoma Protein Dependent

doi:10.1128/MCB.20.12.4210-4223.2000

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Flatt, P. M.
	Articles by Pietenpol, J. A.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Flatt, P. M.
	Articles by Pietenpol, J. A.

Previous Article | Next Article

Molecular and Cellular Biology, June 2000, p. 4210-4223, Vol. 20, No. 12
0270-7306/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

p53 Regulation of G₂ Checkpoint Is Retinoblastoma Protein Dependent

Patricia M. Flatt, Luo Jia Tang, Caroline D. Scatena, Suzanne T. Szak, and Jennifer A. Pietenpol^*

Department of Biochemistry, Center in Molecular Toxicology, and Vanderbilt-Ingram Cancer Center, Vanderbilt University School of Medicine, Nashville, Tennessee 37232

Received 30 September 1999/Returned for modification 10 November 1999/Accepted 15 March 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

In the present study, we investigated the role of p53 in G₂ checkpoint function by determining the mechanism by which p53prevents premature exit from G₂ arrest after genotoxic stress.Using three cell model systems, each isogenic, we showed thateither ectopic or endogenous p53 sustained a G₂ arrest activatedby ionizing radiation or adriamycin. The mechanism was p21 andretinoblastoma protein (pRB) dependent and involved an initialinhibition of cyclin B1-Cdc2 activity and a secondary decreasein cyclin B1 and Cdc2 levels. Abrogation of p21 or pRB functionin cells containing wild-type p53 blocked the down-regulationof cyclin B1 and Cdc2 expression and led to an accelerated exitfrom G₂ after genotoxic stress. Thus, similar to what occurs inp21 and p53 deficiency, pRB loss can uncouple S phase and mitosisafter genotoxic stress in tumor cells. These results indicatethat similar molecular mechanisms are required for p53 regulationof G₁ and G₂checkpoints.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Most human tumors arise from multiple genetic changes which gradually transform growth-limited cells into highly invasivecells that are unresponsive to normal growth controls. The geneticevolution of normal cells into cancer cells is largely determinedby the fidelity of DNA replication, repair, and division (40).Cell cycle arrest in response to DNA damage is an important mechanismfor maintaining genomic integrity. The control mechanisms thatrestrain cell cycle transition after DNA damage are comprisedof multiple signaling pathways and are known as cell cycle checkpoints(17). In normal tissue homeostasis, cells arrest after dissipationof essential growth factors, hormones, or nutrients or if differentiationis induced. After stress, cells arrest at checkpoints either tostall the initiation of DNA synthesis and cell division untilcellular damage can be repaired or to activate pathways that leadtoapoptosis.

It has become increasingly evident that loss of G₁/S checkpoint function is a hallmark of human cancers. If one considersthe frequency of alterations in p53, retinoblastoma protein (pRB),and their upstream regulatory pathways in cancer cells, the majorityof human carcinomas have defective G₁/S checkpoint function. Ofall the genetic alterations identified in human tumors that leadto deregulation of G₁/S checkpoint function, p53 gene mutationis the most common (24). p53 is a short-lived protein presentat very low levels in the nuclei of normal cells; however, a varietyof cellular insults, including DNA damage (27), hypoxia (15),aberrant oncogenic signaling (32), and inhibition of microtubuledynamics (51), result in elevated levels of the protein. p53is a sequence-specific transcription factor (12, 29, 41)that induces expression of several target genes, including p21,Bax, and MDM2 (reviewed in reference 2). Through transactivationof p21, p53 is one of the major regulators of the G₁/S checkpointin response to cellular stress. p21 binds to G₁ cyclin-cyclin-dependentkinase (Cdk) complexes and inhibits their ability to phosphorylatepRB (16). pRB acts as a transcriptional repressor in its hypophosphorylatedstate when it is bound to the E2F family of transcription factors(48). The E2F family mediates transcription of genes requiredfor DNA synthesis, including cyclin E, cyclin A, dihydrofolatereductase, and thymidine kinase (reviewed in reference 57).The binding of hypophosphorylated pRB to E2F has been shown toinhibit E2F-dependent transcription of S-phase genes and arrestcells at the G₁/S transition (22, 47).

Relative to p53's role in G₁ checkpoint responses, a role for p53 in G₂ cell cycle arrest is less well defined. Cells thatdo not contain wild-type p53 are deficient for G₁/S checkpointresponse (33, 49), although the ability of these cells toundergo a G₂ arrest remains intact (31, 33). However, ectopicexpression of p53 in the absence of damage is sufficient to inducecell cycle arrest at both the G₁/S and G₂/M transitions (1,50) and is accompanied by reduced levels and/or differentialsubcellular localization of cyclin B1 protein (25, 60). Recentstudies suggest that p53, p21, and 14-3-3 $sigma$ are necessary to maintaina G₂ arrest following DNA damage, since tumor cells lacking theseproteins enter mitosis with accelerated kinetics (5, 7).Taken together, these results suggest that p53 is not requiredfor the activation of a G₂ arrest in response to genotoxic stressbut that it may dictate the duration of G₂ arrest through p21transactivation.

The goal of this study was to further investigate the role of p53 in G₂ checkpoint function by determining the mechanism bywhich p53 sustains G₂ arrest after genotoxic stress. Three cellculture model systems, each isogenic, were used to show that p53sustains the duration of G₂ arrest after treatment of cells withionizing radiation (IR) or adriamycin (ADR). The p53-mediatedmaintenance of G₂ arrest appears to be dependent on an initialinhibition of the cyclin B1-Cdc2 activity by p21 and a secondarydecrease in cyclin B1 and Cdc2 transcription that is p21 and pRBdependent.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

p53-inducible system. The ecdysone-inducible expression system (Invitrogen, Carlsbad, Calif.) was used to generate cell lines that conditionallyexpress p53. A human hemagglutinin-tagged p53 cDNA was ligatedinto the pIND vector. The resulting vector, pIND-p53, was cotransfectedwith the pVgRXR vector into the human large cell lung carcinomacell line H1299, which is null for p53 expression. Stable cloneswere selected by limiting dilution in F-12 medium containing 10%fetal calf serum (FCS) (Gemini Bio-Products, Inc., Calabasas,Calif.), 1% penicillin-streptomycin (Sigma, St. Louis, Mo.), 600µg of G418 (Mediatech, Herndon, Va.) per ml, and 400 µg of Zeocin(Cayla, Toulouse, France) per ml, and resulting cell lines werenamed H1299-inducible p53 (HIp53). Optimal p53 expression wasobserved after treatment of cells with the ecdysone analog ponasteroneA (PonA) (Invitrogen) at a 10 µM concentration. In all of theexperiments shown, PonA was readministered in fresh medium every24 h to ensure that gene expression was maintained for the durationof theexperiment.

Cell culture and treatment. The RKO-E7 and RKO-NEO cell lines, kindly provided by K. Cho (University of Michigan, Ann Arbor), were cultured in McCoy's5A medium (Gibco BRL, Gaithersburg, Md.) supplemented with 10%FCS 1% penicillin-streptomycin, and 500 µg of G418 per ml. Thehuman colorectal carcinoma cell line HCT116 and the isogenic derivativelines HCT116 p53^/ and HCT116 p21^/ were kindly provided by B. Vogelstein (Johns Hopkins OncologyCenter, Baltimore, Md.) and cultured in McCoy's 5A medium supplementedwith 10% FCS and 1% penicillin-streptomycin. Cells were treatedwith ADR or IR as indicated in the figures. IR was delivered atroom temperature with a ¹³⁷Cs irradiator (J. L. Shepherd and Associates). All cells werecultured at 37°C with 5% CO₂.

Fluorescence-activated cell sorter analysis. Approximately 10⁶ cells were incubated with 20 µg of propidium iodide (Sigma) per ml, and DNA content was determined usinga FACS Caliber (Becton Dickinson). Data were plotted using CellQuestsoftware, and axis scales were optimized using the control sampleand were maintained at that value throughout each experiment.Fifteen thousand events were analyzed for each sample. Bromodeoxyuridine(BrdU) incorporation was performed and analyzed as previouslydescribed (13).

Western blot analysis and immunoprecipitations. Cells were trypsinized, washed twice with ice-cold phosphate-buffered saline, and harvested in kinase lysis buffer (KLB) (50mM Tris-HCl [pH 7.4], 150 mM NaCl, 0.1% Triton X-100, 0.1% NonidetP-40, 4 mM EDTA, 50 mM NaF, 0.2 mM Na vanadate) containing theprotease inhibitors antipain (10 µg/ml), leupeptin (10 µg/ml),pepstatin A (10 µg/ml), chymostatin (10 µg/ml) (Sigma), and 4-(2-aminoethyl)-benzenesulfonylfluoride(200 µg/ml) (Calbiochem-Novabiochem Corp., La Jolla, Calif.).Cells were lysed by passage through a 23-gauge needle, and theprotein supernatant was clarified by centrifugation at 13,000× g for 10 min at 4°C. Protein concentration was determined bythe Bradford protein assay (Bio-Rad Laboratories, Inc., Hercules,Calif.). Western blot analysis was performed as previously described(13) using the following primary antibodies: anti-p53 polyclonalantibody 1801 (Oncogene Research Products, Calbiochem, Cambridge,Mass.), anti-p21 antibody Waf1/Cip1 EA10 (Oncogene Research Products),anti-MDM2 antibody SMP14 (Santa Cruz Biotechnology Inc., SantaCruz, Calif.), anti-Cdc2 antibody 17 (Santa Cruz BiotechnologyInc.), anti-cyclin B1 antibody GNS1 (Santa Cruz BiotechnologyInc.), anti-pRb antibody LM95.1 (Oncogene Research Products),and anti-Bax antibody N-20 and anti-Actin antibody I-19 (SantaCruz Biotechnology). In all Western blot analyses, uniform proteinloading was confirmed by fast green staining. For immunoprecipitation-basedexperiments, anti-cyclin B1 GNS1, anti-Cdc2 17, and anti-p21 EA10antibodies were cross-linked to protein G-Sepharose (PharmaciaBiotech Products, Piscataway, N.J.) as previously described (52).HIp53 cells were treated as indicated in the figure legends andharvested in KLB as described above. Cell lysates (500 µg) wereimmunoprecipitated with cross-linked antibody for 2 h at 4°C withrocking. Immunoprecipitated proteins were washed three times inKLB, resuspended in 1× Laemmli sample loading buffer, heated at85°C for 10 min, and analyzed by Westernblotting.

Kinase assays. Kinase assays were performed as previously described (13). Cell lysates (250 µg) were immunoprecipitated with anti-Cdk2antibody M2 (Santa Cruz Biotechnology Inc.) or anti-cyclin B1antibody GNS1 (Santa Cruz Biotechnology Inc.). The kinase assaywas initiated by adding 2 µCi of [ $gamma$ -³²P]ATP (3,000 Ci/mmol) (New England Nuclear Laboratories) and incubatedat 30°C for 10 min using 7 µg of histone H1 (Boehringer Mannheim,Indianapolis, Ind.) as a substrate. The reaction was terminatedby the addition of 25 µl of 2× Laemmli sample loading buffer.Reaction mixtures were heated at 85°C for 10 min and subjectedto sodium dodecyl sulfate (SDS)-12% polyacrylamide gel electrophoresis.³²P-labeled histone H1 was quantified on an Instant Imager (Packard,Meriden, Conn.).

Northern blot analysis. Cells were harvested in RNA lysis buffer (10 mM Tris [pH 7.5], 100 mM NaCl, 2 mM EDTA, 1% SDS) and lysed by passage througha 23-gauge needle eight times. Proteinase K was added to the lysateto a final concentration of 100 µg/ml, and the lysate was incubatedat 37°C for 1 h. Following proteinase K digestion, the NaCl concentrationwas adjusted to 400 mM. The samples were heated at 65°C for 5min with constant agitation, followed by immediate cooling inice water for 30 s. mRNA was isolated by incubation with oligo(dT)cellulose (Ambion Inc., Austin, Tex.) with rocking at room temperaturefor 2 h. The RNA-oligo(dT) cellulose mixture was washed twicewith high-salt buffer (10 mM Tris [pH 7.5], 400 mM NaCl, 1 mMEDTA, 0.2% SDS) and packed with high-salt buffer on a poly prepchromatography column (Bio-Rad Laboratories, Inc.). The columnwas washed once with high-salt buffer and once with low-salt buffer(10 mM Tris [pH 7.5], 100 mM NaCl, 1 mM EDTA, 0.2% SDS). The mRNAwas eluted from the column with 55°C elution buffer (5 mM Tris[pH 7.5], 1 mM EDTA, 0.2% SDS). mRNA was precipitated at $-$ 20°Covernight with the addition of sodium acetate (pH 5.2) to a finalconcentration of 220 mM and two volumes of 95% ethyl alcohol.After precipitation, mRNA was recovered by centrifugation at 12,000× g for 30 min and the pellet was rinsed once with 70% ethyl alcohol.The pellet was dried by inversion at room temperature and resuspendedin sterile H₂O. RNA (5 µg) was lyophilized, resuspended in samplebuffer {1× morpholinepropanesulfonic acid (MOPS; 0.1 M MOPS [pH7.0], 40 mM sodium acetate, 5 mM EDTA [pH 8.0]), 50% formamide,6.5% formaldehyde} and heated at 55°C for 15 min. A 10× loadingbuffer (50% glycerol, 1 mM EDTA, 0.25% bromophenol blue, 0.25%xylene cyanol, 0.3 mg of ethidium bromide per ml) was added tothe sample at a 1× concentration, and mRNA was resolved by gelelectrophoresis on a 1% agarose gel containing 2% formaldehydeand 1× MOPS. The gel was washed twice in 10× SSC (1× SSC is 0.15M NaCl plus 0.015 M sodium citrate) buffer, and mRNA was transferredto a supported nitrocellulose membrane (Gibco BRL). Cyclin B1and Cdc2 cDNAs were labeled with [ $alpha$ -³²P]dCTP using Rediprime II (Amersham). Cyclin B1 cDNA was kindlyprovided by E. Nishida (Kyoto University, Kyoto, Japan), and Cdc2cDNA was kindly provided by H. Piwnica-Worms (Washington University,St. Louis, Mo.). After a 2-h prehybridization in Express Hyb (ClontechLaboratories, Inc., Palo Alto, Calif.), membranes were incubatedwith 2 × 10⁶ cpm of labeled cDNA per ml in Express Hyb at 42°C overnight.Membranes were washed twice at room temperature in 2× SSC-0.1%SDS, followed by two washed in 0.2× SSC-0.1% SDS at 42°C.

Electrophoretic mobility shift assays (EMSA). After treatment as indicated above, either HIp53, HCT116, HCT116 p53^/, or HCT116 p21^/ cells were harvested in microextraction buffer (20 mM HEPES [pH7.8], 450 mM NaCl, 0.2 mM EDTA, 0.5 mM dithiothreitol, 25% glycerol)and sonicated. Protein supernatants were clarified by centrifugation,frozen in a methanol-dry-ice bath, and stored at $-$ 80°C until processed.An oligonucleotide duplex containing a consensus E2F binding sitefrom the human c-myc promoter (23) was labeled with the Klenowfragment using [ $alpha$ -³²P]dATP for 30 min at 37°C. Labeled oligonucleotide was purifiedby phenol-chloroform extraction and ethanol precipitation andresuspended in H₂O. Gel shift reactions were performed by incubating15 µg of protein lysate in 1× binding buffer (100 mM HEPES [pH7.9], 5 mM MgCl₂, 0.4 mM EGTA, 2 mM dithiothreitol, 200 mM KCl),5% Ficoll, 200 ng of salmon sperm DNA, and 100,000 cpm of labeledoligonucleotide for 20 min at room temperature. For supershiftassays, 1 µg of anti-Rb antibody IF8 (Santa Cruz Biotechnology,Inc.) was added per reaction mixture 5 min after the start ofthe 20-min incubation. For competition reactions, either a 25-,50-, or 100-fold excess of unlabeled oligonucleotide was addedto the reaction mixtures prior to the addition of protein lysate.Binding was resolved on a 4% acrylamide gel in 0.25× Tris-borate-EDTA.

CAT assays. HIp53 cells were transiently transfected with pCAT-cyclin B1 or a pCAT vector control (25) using Lipofectamine (Gibco BRL)and treated with ADR 24 h after transfection. The chloramphenicolacetyltransferase (CAT) vectors were kindly provided by J. Lee(Hamilton Regional Cancer Center, Hamilton, Ontario, Canada).After 17 h of ADR treatment, the ADR was removed and the cellswere washed twice with phosphate-buffered saline and culturedin the presence or absence of 10 µM PonA for 24 and 48 h. Cellswere harvested in 0.25 M Tris, pH 7.8, and lysed by three cyclesof freezing and thawing. Supernatants were clarified by centrifugationat 12,000 × g and stored at $-$ 80°C until assayed. Protein concentrationwas determined by the Bradford assay, and 75 µg of protein wasused to determine CAT activity using acetyl coenzyme A as a substratefor chloramphenicol-D-threo-[dichloroacetyl-1,2-¹⁴C] ([¹⁴C]CAP) incorporation. Protein lysate was incubated with 5 µl of[¹⁴C]CAP (0.05 µCi/ml) and 450 µM acetyl coenzyme A for 40 min at37°C. The reaction was terminated by the addition of 4°C ethylacetate. Reaction mixtures were centrifuged at 12,000 × g for2 min, and the upper layer was removed and dried under vacuum.Samples were resuspended in ethyl acetate, spotted onto thin-layerchromatography plates (J. T. Baker, Inc., Phillipsburg, N.J.),and resolved by ascending thin-layer chromatography in chloroform-methanol(95:5) until the solvent front was 1 cm from the top of theplate.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

p53 expression sustains genotoxic stress-induced G₂ growth arrest. To determine the mechanism by which p53 regulates the G₂ checkpoint response, we used three cell culture model systems: (i)a cell line that conditionally expresses ectopic p53; (ii) anisogenic set of HCT116 colorectal carcinoma cell lines that consistsof the parental line, which endogenously expresses wild-type p53,and two derivative lines, HCT116 p53^/ (5) and HCT116 p21^/ (54), which are null for p53 and p21, respectively; and (iii)a pair of RKO colorectal carcinoma cell lines, the parental line,and an E7-expressing line, RKO-E7 (49).

For the first line of experimentation, we developed a cell line that would conditionally express p53. A human lung carcinomacell line (H1299) that is null for the endogenous expression ofp53 was stably transfected with an ecdysone-inducible p53 expressionvector. The resulting cell line, HIp53, was derived. After treatmentof HIp53 cells with the ecdysone analog PonA, p53 protein levelsincreased in a dose-dependent manner. Optimal induction of p53was achieved with a PonA dose of 10 µM (data not shown), and thisconcentration was used in the experiments whose results are shown.By 8 h after PonA treatment, p53, MDM2, and p21 proteins weredetectable. Both MDM2 and p21 protein levels remained elevatedthrough 48 h, while a decrease in p53 protein levels occurredby 48 h (Fig. 1A). MDM2 has been shown to mediate the degradationof p53 (18, 30), and thus the decline in p53 levels by 48h of PonA treatment may be due in part to the continual inductionof MDM2 (Fig. 1A). Treatment of a vector control cell line (H10)with PonA did not result in an increase in p21 or MDM2 proteinin the absence of p53 (Fig. 1A).

View larger version (45K):
[in this window]
[in a new window]

FIG. 1. Ectopic expression of p53 leads to reversible G₁ and G₂ growth arrest. HIp53 cells were treated with PonA for 48 h, the analog was removed, and cells were grown for an additional 72 h. (A) HIp53 cells were harvested at 8, 24, and 48 h following PonA addition and after PonA removal. Protein lysates were analyzed by Western blotting for the indicated proteins. (B) Simultaneous flow cytometric analyses for DNA synthesis (BrdU incorporation) and DNA content (propidium iodide staining) were performed at the indicated times. Results are representative of three independent experiments. Con, control.

To determine the cell cycle distribution and proliferative capacity of HIp53 cells in the absence of damage, simultaneousflow cytometric analyses for DNA synthesis (BrdU incorporation)and DNA content (propidium iodide staining) were performed (Fig.1B). For these experiments, HIp53 cells were treated with PonAfor 48 h, the analog was removed, and cells were grown for anadditional 48 h. During each 24-h interval after PonA treatmentand removal, cells were incubated with BrdU for 2 h prior to harvest(Fig. 1B). As evidenced by the flow cytometric histogram profileand the 28-fold decrease in BrdU incorporation, the HIp53 cellsunderwent cell cycle arrest at both G₁ and G₂ after 48 h of PonAtreatment (Fig. 1B) while treatment of HI0 with PonA did not inducea cell cycle arrest or a decrease in BrdU incorporation (datanot shown). After PonA removal, HIp53 cells reentered the cellcycle, as was confirmed by a 56-fold increase in BrdU incorporationat 24 h (Fig. 1B). Reentry of HIp53 cells into the cycle afterremoval of PonA was followed by a rapid decrease in p53 levels(Fig. 1A). Parallel decreases in MDM2 and p21 protein levels werealso observed (Fig. 1A). Thus, in the absence of cellular stress,ectopic expression of p53 arrested HIp53 cells in the G₁ and G₂phases of the cellcycle.

To determine if p53 expression affected the duration of G₂ arrest after stress, HIp53 cells were treated with either IR orADR prior to the induction of p53 with PonA. Treatment of HIp53cells with IR (8, 12, 20, or 30 Gy) resulted in an accumulationof cells with a 4 N DNA content by 15 h (Fig. 2A and Table 1).After the IR-induced G₂ arrest at 15 h, the HIp53 cells were culturedin the presence or absence of PonA for an additional 24, 48, or72 h. The G₂ arrest induced after exposure to 8 or 12 Gy of IRwas transient, and p53 expression had only a minimal effect onthe duration of the arrest. However, exposure of the cells tohigher doses of IR (20 or 30 Gy) increased the length of G₂ arrestand expression of p53 sustained the G₂ arrest through the timecourse examined (Fig. 2A and Table 1). In the absence of p53expression, cells did not maintain the cell cycle arrest; rather,a majority lost viability and detached from the plate by 48 and72 h after exposure to IR, thus accounting for the diminishedpeaks in the histograms seen in Fig. 2A at those times.

View larger version (16K):
[in this window]
[in a new window]

FIG. 2. p53 prolongs G₂ cell cycle arrest after exposure to IR or ADR. Cells were harvested at the indicated times and analyzed by flow cytometric analysis. (A) Cells were treated with IR (8, 12, 20, and 30 Gy) and incubated for 15 h, after which time cells were cultured for an additional 24, 48, or 72 h in the presence or absence of PonA. (B) Cells were treated with ADR (90, 175, 350, or 525 nM) for 17 h, the drug was washed out, and the cells were cultured for an additional 24, 48, or 72 h in the presence or absence of PonA. Fifteen thousand events were analyzed for each condition, and all histograms were plotted by using the same scale for both axes. Results are representative of two independent experiments.

View this table:
[in this window]
[in a new window]

TABLE 1. Cell cycle distribution of HIp53 cells after IR

HIp53 cells were also treated with ADR (dose range, 90 to 525 nM) for 17 h, the drug was washed out, and the cells were culturedin the presence or absence of PonA for an additional 24, 48, or72 h. ADR treatment induced a dose-dependent G₂ arrest in HIp53cells, with the highest percentage of cells arresting with a 4N DNA content after treatment with 350 and 525 nM ADR (Fig. 2Band Table 2). At all of the ADR doses tested, the expressionof p53 increased the duration of time that cells remained arrestedin both the G₁ and G₂ phases of the cell cycle compared to arresttimes for cells lacking p53 (Fig. 2B and Table 2). The most pronouncedp53-mediated maintenance of G₂ arrest occurred 48 and 72 h aftertreatment with 350 and 525 nM ADR (Fig. 2B and Table 2). In contrast,the majority of the cells lacking p53 expression did not maintainthe cell cycle arrest, lost viability, and detached from the plateby 48 and 72 h after exposure to ADR, thus accounting for thediminished frequencies in the histograms seen in Fig. 2B at thosetimes. Thus, after exposure of HIp53 cells to IR or ADR, p53 significantlyextended the period of G₂ arrest compared with that of cells deficientfor p53.

View this table:
[in this window]
[in a new window]

TABLE 2. Cell cycle distribution of HIp53 cells after ADR treatment

To verify and extend the observations described above, we also analyzed the role of p53 in G₂ checkpoint response in an isogenicset of HCT116 colorectal carcinoma cell lines. HCT116, HCT116p53^/, and HCT116 p21^/ cells were treated with IR or ADR and analyzed for DNA contentby flow cytometry at 24, 48, 72, and 96 h (in the case of ADR)after treatment. Twenty-four hours after treatment with IR orADR, all of the HCT116-derived cell lines had an accumulationof cells with, predominantly, a 4 N DNA content (Fig. 3A). However,by 72 h after treatment with either genotoxic agent, the HCT116p53^/ and the HCT116 p21^/ cells had reductions in the numbers of cells with a 4 N DNA contentcompared with the numbers for the parental HCT116 cells (Fig.3B).

View larger version (29K):
[in this window]
[in a new window]

FIG. 3. p21 is required for regulation of G₂ checkpoint arrest. HCT116, HCT116 p53^/, and HCT116 p21^/ cells were treated with IR (8 Gy) or ADR (350 nM) and analyzed 24, 48, and 72 h after treatment. (A and B) Cells were analyzed by flow cytometric analysis. (A) Propidium iodide fluorescence profile for control (Con) and 24-h time points; (B) quantifications from the flow histograms presented as percentages of cells with a 4 N DNA content after treatment with IR or ADR. Fifteen thousand events were analyzed for each condition, and all histograms were plotted by using the same scale for both axes. Results are representative of two independent experiments.

In order to compare the findings above and subsequent molecular results obtained with the two different cell model systems,we determined the relative levels of p53 in each cell line beforeand after ADR treatment. HIp53 and HCT116 cells were treated withADR (350 nM) for 17 h, the drug was removed, and the cells weregrown in fresh growth medium. With the HIp53 cells, PonA was addedafter 17 h to induce p53. For each line, the same number of cells(500,000) was harvested from control and treated cultures andprotein lysates were prepared and analyzed on the same Westernblot for p53 protein levels (Fig. 4). Relative to levels in theHIp53 cells, the HCT116 cells had higher levels of p53 proteinat each time analyzed after ADR treatment. The slower migrationof the p53 protein in the HIp53 cells was due to the inclusionof a hemagglutinin tag at the 5' end of the p53 protein. The comparisonof p53 levels in the two cell lines assured us that results obtainedwith the HIp53 cells were not due merely to the higher levelsof overexpressed p53 protein, as is the concern with many ectopicexpression systems.

View larger version (33K):
[in this window]
[in a new window]

FIG. 4. Relative levels of p53 protein in HCT116 and HIp53 cells. HIp53 and HCT116 cells were treated with ADR (350 nM) for 17 h, the drug was removed, and the cells were grown in fresh growth medium. With the HIp53 cells, PonA was added after 17 h to induce p53. For each line, the same number of cells (500,000) was harvested from control (Con) and treated cultures and protein lysates were prepared and analyzed on the same Western blot for p53 protein levels. Actin analysis was included to assess protein loading and transfer. Results are representative of three independent experiments.

p53 expression results in loss of cyclin B1-Cdc2 activity. To elucidate the mechanism underlying the prolonged stress-induced G₂ arrest observed in the cells containing an intact p53signaling pathway, we examined proteins known to play a role inthe regulation of G₂ transition. Progression of cells from G₂to mitosis requires the activity of the cyclin B1-Cdc2 complex(34). When cells undergo genotoxic stress, the activity of thiscomplex is reduced through inhibitory phosphorylations of Cdc2and cells arrest in G₂ (36, 38). p21 is increased in a p53-dependentmanner and can bind and inhibit the activities of several Cdks,including cyclin B1 and Cdc2 (16). We hypothesized that theobserved p53 regulation of the G₂ checkpoint was mediated throughinhibition of cyclin B1-Cdc2 activity. To test this hypothesis,protein lysates were prepared from the cells described in thelegends to Fig. 2 and 3 and processed using Western blot- andimmunoprecipitation-basedassays.

In the HIp53 cells, an increase in p21 protein occurred in cells that expressed p53 while only low-level p21 protein was detectablein IR- or ADR-treated cells lacking p53 (Fig. 5A and B). At alldoses of IR or ADR tested, significant reductions in cyclin B1and Cdc2 protein levels were observed by 48 and 72 h after inductionof p53 (Fig. 5A and B). The cell cycle arrest pattern of the cellsvaried with the dose of the genotoxic agent (Fig. 2); however,the observed reduction of cyclin B1 and Cdc2 protein at 72 h wasindependent of cell cycle position. Of note, the kinetics of cyclinB1 protein loss were more rapid at lower doses and correlatedwith a greater number of cells arrested in G₁. In contrast, cellstreated with IR or ADR that lack p53 expression had an increasein cyclin B1 and Cdc2 protein levels at all doses examined.

View larger version (42K):
[in this window]
[in a new window]

FIG. 5. p53 expression after IR or ADR inhibits cyclin B1-Cdc2 kinase activity. (A) Cells were treated with IR (8, 12, and 20 Gy) and incubated for 15 h, after which time cells were cultured for an additional 24, 48, or 72 h in the presence or absence of PonA. Protein lysates were analyzed by Western blotting for the indicated proteins. (B) Cells were treated with ADR (90, 175, 350, or 525 nM) for 17 h, the drug was washed out, and the cells were cultured an additional 24, 48, or 72 h in the presence or absence of PonA. (C and D) Protein lysates were analyzed by cyclin B1 immunoprecipitation-based assays for Cdc2 kinase activity using histone H1 as a substrate (C) and for immunoprecipitable cyclin B1, Cdc2, and p21 proteins by Western blotting (D). HIp53 cells were treated with 525 nM ADR for the data presented in panels C and D. Results are representative of two independent experiments. Con, control; IP, immunoprecipitation.

Accompanying the reduction in cyclin B1 and Cdc2 protein levels in the HIp53 cells, we observed a 60% decrease in cyclin B1-Cdc2activity by 24 h after p53 induction and a further decline to10% of control levels by 72 h (Fig. 5C). Conversely, in the absenceof p53 expression there was an increase in cyclin B1-Cdc2 activitythrough 48 h, with levels elevated 6.5-fold higher than that ofthe control (Fig. 5C). At 24 h after ADR removal, the decreasein cyclin B1-Cdc2 kinase activity in HIp53 cells expressing p53(Fig. 5C) preceded any marked decrease in cyclin B1 and Cdc2 proteinlevels (Fig. 5B). In addition, the loss of cyclin B1-Cdc2 kinaseactivity 24 h after p53 induction did not correlate with inhibitoryphosphorylation of Cdc2, as the predominant form of the proteinwas in the faster-migrating, hypophosphorylated state (Fig. 5B).

We hypothesized that the initial down-regulation of cyclin B1-Cdc2 kinase activity 24 h after p53 induction was due to thedirect association of p21 with the cyclin B1-Cdc2 complex. Totest this hypothesis, protein lysates were immunoprecipitatedwith cyclin B1 antibodies and analyzed by Western blotting forcyclin B1, Cdc2, and p21. Both p21 and Cdc2 coimmunoprecipitatedwith cyclin B1 24 h after p53 expression in ADR-treated HIp53cells (Fig. 5D). Consistent with the decrease in cyclin B1 levelsseen in Fig. 5B, the levels of immunoprecipitable cyclin B1, aswell as those of any coimmunoprecipitable Cdc2 and p21, were reducedby 72 h after p53 expression (Fig. 5D). p21 was not coimmunoprecipitatedwith cyclin B1 in ADR-treated cells that lacked p53 expression;however, increasing amounts of Cdc2 coprecipitated with cyclinB1 at 24, 48, and 72 h in the absence of p53 expression. Thus,the maintenance of G₂ arrest in cells expressing p53 after genotoxicstress appears to involve a two-step mechanism, including an initialinhibition of cyclin B1-Cdc2 activity through p21 associationwith the complex, followed by a marked decrease in cyclin B1 andCdc2 proteinlevels.

In both HCT116 and HCT116 p21^/ cells, p53 levels increased and remained elevated through 72 h after IR (Fig. 6A). Similar changesin p53 levels were observed after ADR treatment (Fig. 6B). p21protein levels were significantly elevated only in HCT116 cellsafter IR and ADR treatment (Fig. 6A and B). p53-independent elevationof p21 protein was also observed in the HCT116 p53^/ cells. There was a decrease in cyclin B1 and Cdc2 protein levelsby 24 h in HCT116 cells exposed to both IR and ADR, while cyclinB1 and Cdc2 protein levels remained elevated in HCT116 p53^/ and HCT116 p21^/ cells (Fig. 6A and B). Similar to the results for the HIp53 cells,we observed a 60% decrease in cyclin B1-Cdc2 activity by 24 hafter ADR treatment and a further decline to 10% of control levelsby 72 h in the HCT116 cells (Fig. 6C). Conversely, in the absenceof a functional p53 signaling pathway in the HCT116 p53^/ and HCT116 p21^/ cells, there was an increase in cyclin B1-Cdc2 activity through72 h, with levels elevated 1.3- to 2-fold higher than that ofthe control (Fig. 6C). These data are consistent with the resultsobtained with the HIp53 cells and support the hypothesis thatp53 regulation of the G₂ checkpoint occurs through a p21-dependentmechanism that involves a reduction of cyclin B1 and Cdc2 proteinlevels.

View larger version (50K):
[in this window]
[in a new window]

FIG. 6. p21 is required for p53-mediated loss of cyclin B1 and Cdc2 protein levels. Cells were treated as described in the legend to Fig. 3 with IR (A) or ADR (B), harvested, and analyzed by Western blotting for the indicated proteins. Actin analysis was included to assess protein loading and transfer. (C) Protein lysates were analyzed by cyclin B1 immunoprecipitation-based assays for Cdc2 kinase activity using histone H1 as a substrate. Results are representative of three independent experiments. C and Con, control.

Loss of cyclin B1 and Cdc2 after p53 expression is due to a reduction in cyclin B1 and Cdc2 mRNA. To determine whether the p53-dependent decrease in cyclin B1 and Cdc2 protein levels was due to a reduction in cyclin B1 andCdc2 mRNA, Northern blot analyses were performed. A time-dependentloss of cyclin B1 and Cdc2 mRNA was observed in ADR-treated HIp53cells and in HCT116 cells that expressed p53 (Fig. 7A and B).In both cell lines, the levels of cyclin B1 and Cdc2 mRNA werereduced by 70 to 90% by 72 h (Fig. 7A and B). These results areconsistent with the observed decrease in cyclin B1 and Cdc2 proteinlevels (Fig. 5B and 6B). In contrast, cyclin B1 and Cdc2 mRNAlevels were elevated at 24 and 48 h after ADR treatment in cellsthat lacked an intact p53 signaling pathway (Fig. 7A and B). Tofurther extend these results, a cyclin B1 promoter-CAT reportervector (pCAT-cyclin B1) was transfected into the HIp53 cells.The cells were treated with ADR for 17 h, the drug was washedout, and the cells were cultured for an additional 24 or 48 hin the presence or absence of PonA. Induction of p53 after ADRtreatment resulted in a 4.5-fold reduction in cyclin B1 promoter-CATactivity by 48 h compared with the CAT activity in cells lackingp53 (Fig. 7C). Taken together, these data suggest that the lossof cyclin B1 and Cdc2 protein observed during p53-mediated sustainedG₂ arrest was due to decreases in cyclin B1 and Cdc2 mRNA levelsand that the regulation of cyclin B1 occurred at the transcriptionallevel.

View larger version (34K):
[in this window]
[in a new window]

FIG. 7. Loss of cyclin B1 and Cdc2 expression after p53 expression. (A) HIp53 cells were treated with 525 nM ADR for 17 h, the drug was washed out, and the cells were cultured in the presence or absence of PonA for 24, 48, or 72 h. Cells were harvested, mRNA was isolated, and Northern blot analyses were performed for cyclin B1 or Cdc2 mRNA. (B) HCT116 and HCT116 p53^/ cells were treated with 350 nM ADR for the times indicated, and cells were harvested, mRNA was isolated, and Northern blot analyses were performed for cyclin B1 and Cdc2. (C) HIp53 cells were transfected with either pCAT-cyclin B1 or with the pCAT vector. Twenty-four hours after transfection, the cells were treated with 525 nM ADR. The drug was washed out 17 h after treatment, and the cells were cultured an additional 24 or 48 h in the presence or absence of PonA. Cells were harvested and analyzed for CAT activity. Results are representative of two independent experiments. Con, control; EtBr, ethidium bromide.

Cyclin B1 and Cdc2 transcription is dependent on the activity of cyclin A-Cdk2 complexes in late S phase (35). Furthermore,the expression of Cdc2 and cyclin A are regulated by the E2F familyof transcription factors (8, 9, 14, 46). We hypothesizedthat the p53-mediated inhibition of cyclin B1 transcription wasdependent on p21 inhibition of cyclin-Cdk complexes, the resultinghypophosphorylation of pRB, and subsequent inhibition of an E2F-dependenttranscriptional cascade. To test this hypothesis, we analyzedADR-treated HIp53 and HCT116 cells for Cdk2 activity and pRB phosphorylationstate. Cdk2 activity was significantly inhibited by 24 h in theHIp53 and HCT116 cell lines and completely inhibited by 72 h inthe HIp53 cells and by 90% in the HCT116 cells (Fig. 8). In contrast,cells without an intact p53 signaling pathway displayed a 1.5-to 3-fold increase in Cdk2 activity over the time course (Fig.8). Analysis of pRB phosphorylation revealed that pRB was predominantlyin the hyperphosphorylated, inactive state in HIp53 cells lackingp53 expression as well as the HCT116 p21^/ cells but was predominantly in the hypophosphorylated, activestate in ADR-treated HIp53 and HCT116 cells expressing p53 andp21 (Fig. 8). Faster-migrating forms of pRB were detectable inHCT116 p53^/ cells and were likely due to the p53-independent elevation ofp21 protein (Fig. 6B) that occurred after ADR treatment; however,these forms were not sufficient to inhibit cyclin B1-Cdc2 or Cdk2activity (Fig. 6C and 8B). These results led to the hypothesisthat in the presence of p53, there is a pRB-dependent inhibitionof E2F transcriptional activity in G₂-arrested cells.

View larger version (61K):
[in this window]
[in a new window]

FIG. 8. Dephosphorylation of pRB during p53 regulation of the G₂ checkpoint. (A) HIp53 cells were treated with 525 nM ADR for 17 h, the drug was washed out, and the cells were cultured for the indicated times in the presence or absence of PonA. (A) Cells were harvested and analyzed by Western blot analysis for pRB protein levels and phosphorylation state (upper blot) and for Cdk2 kinase activity using histone H1 as a substrate (lower blot). (B) HCT116, HCT116 p53^/, and HCT116 p21^/ cells were treated with 350 nM ADR for the times indicated, and the cells were harvested and analyzed by Western blot analysis for pRB protein levels and phosphorylation state (upper blot) and for Cdk2 kinase activity using histone H1 as a substrate (lower blot). Results are representative of three independent experiments. C and Con, control.

To assess the interaction between pRB and E2F transcription factors, EMSA were performed using an E2F binding element fromthe human c-myc gene (23). Gel shift analyses showed that threedifferent E2F complexes were formed with proteins harvested fromrapidly cycling populations of HIp53, HCT116, and HCT116 p53^/ cells (Fig. 9, complexes a, b, and c). The formation of threeprotein-DNA complexes with this E2F binding element is consistentwith previous observations (23). These three complexes couldbe efficiently competed with excess unlabeled binding site DNA(Fig. 9). In ADR-treated cells that lacked p53 expression, therewere increases in levels of the slower-migrating complex at 24and 48 h (Fig. 9, complex a). In ADR-treated cells expressingp53, slower-migrating complex a was undetectable by 48 h (Fig.9). The decrease in complex a formation was accompanied by anincrease in the intensity of complex b in cells expressing p53.To determine which of these complexes contained pRB, supershiftassays were performed with an antibody specific for pRB. The supershiftanalyses revealed that complex b contained pRB (Fig. 9). The resultsindicate that a significant fraction of the E2F protein is incomplex with pRB in G₂-arrested cells that express p53.

View larger version (55K):
[in this window]
[in a new window]

FIG. 9. pRB interaction with E2F transcription factors in HIp53, HCT116, and HCT116 p53^/ cells after genotoxic stress. An EMSA was performed to analyze pRB and E2F interaction using an E2F binding element derived from the human c-myc promoter. For competition assays, either a 25-, 50-, or 100-fold excess of unlabeled oligonucleotide was added. For supershift assays, 1 µg of anti-pRB antibody was added to reaction mixtures 5 min after the incubation was initiated. Free, oligonucleotide duplex alone. (A) HIp53 cells were treated with 525 nM ADR for 17 h, the drug was washed out, and the cells were cultured for the indicated times in the presence or absence of PonA. Cells were harvested and analyzed. (B) HCT116 and HCT116 p53^/ cells were treated with 350 nM ADR for the times indicated, and the cells were harvested and analyzed. Results are representative of three independent experiments. Con, control; comp., competitor.

Disruption of pRB signaling abrogates the maintenance of G₂ arrest. Based on the results described above, we hypothesized that p53 regulation of G₂ arrest was pRB dependent. To test this hypothesis,we used a set of RKO cells developed by Slebos and colleaguesthat stably express either the human papillomavirus (HPV) type16 E7 protein (RKO-E7) or the vector alone (RKO-NEO) (49). Expressionof the HPV type 16 E7 viral protein abrogates pRB function inthese cells (11, 49, 59). RKO-NEO and RKO-E7 cells weretreated with IR or ADR, and DNA contents were assessed by flowcytometric analysis at 24, 48, and 72 h after exposure to theagents. In both RKO-NEO and RKO-E7 cultures, there was an accumulationof cells with a predominant 4 N DNA content at 24 h after IR and17 h after ADR treatment (Fig. 10A). There was also an arrest ofthe RKO-NEO cells in G₁ that was abrogated by E7 expression (Fig.10A) as previously reported (49). RKO-NEO cells sustained theG₂ arrest after both IR and ADR treatment through 72 h (Fig. 10B),whereas a significant fraction of RKO-E7 cells exited from G₂and endoreduplicated as evidenced by the accumulation of cellswith a 8 N DNA content (Fig. 10A, ADR treatment).

View larger version (38K):
[in this window]
[in a new window]

FIG. 10. pRB is required for prolonged G₂ arrest and loss of cyclin B1 and Cdc2 protein levels. RKO-NEO and RKO-E7 cells were treated with IR (10 Gy) or ADR (350 nM), the drug was washed out at 17 h, and cells were harvested at 24, 48, and 72 h. (A and B) Cells were analyzed by flow cytometric analysis. (A) Propidium iodide fluorescence profile for control (Con) and treated cells; (B) quantifications from the flow histograms presented as percentages of cells with a 4 N DNA content after treatment with IR or ADR. Fifteen thousand events were analyzed for each condition, and all histograms were plotted by using the same scale for both axes. Protein lysates from cells exposed to IR (C) and ADR (D) were analyzed by Western blotting for the indicated proteins. (E) Protein lysates were analyzed for Cdc2 and Cdk2 kinase activities using histone H1 as a substrate. Results are representative of two independent experiments.

Analysis of proteins from the RKO cell lines revealed that p53 and p21 levels increased in similar manners in both RKO-NEOand RKO-E7 lines after both treatments (Fig. 10C and D). CyclinB1 and Cdc2 protein levels were reduced in RKO-NEO cells 72 hafter IR and 48 h after ADR treatment, while RKO-E7 cells maintainedcontrol or higher levels of cyclin B1 and Cdc2 after treatmentwith IR and ADR (Fig. 10C and D). pRB was in the hypophosphorylatedform in RKO-NEO cells between 48 and 72 h after IR and ADR treatment,whereas pRB remained predominantly in the phosphorylated statein RKO-E7 cells (Fig. 10C and D). Dephosphorylation of pRB in RKO-NEOcells occurred with kinetics similar to those seen with the decreasein cyclin B1 and Cdc2 protein levels. Consistent with the reductionin cyclin B1 and Cdc2 proteins levels, we observed a decreasein cyclin B1-Cdc2 and Cdk2 activities in RKO-NEO cells by 72 hafter IR and ADR exposure (Fig. 10E). In contrast, there was anincrease in cyclin B1-Cdc2 and Cdk2 kinase activities after IRand ADR treatment in RKO-E7 cells (Fig. 10E). These biochemicalchanges mirror those observed in the HIp53 and the HCT116 cellsystems and indicate that pRB plays an integral role in p53-mediatedmaintenance of the G₂ arrest after genotoxicstress.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The results presented provide a mechanism for how p53 sustains G₂ arrest after genotoxic stress. Treatment of p53-deficientcells with genotoxic agents induced a transient G₂ arrest thatwas followed by an increase in cyclin B1-Cdc2 kinase activityand premature progression of cells into mitosis, whereas in cellsexpressing p53, G₂ arrest was sustained through an initial inhibitionof cyclin B1-Cdc2 activity, followed by a marked decrease in cyclinB1 and Cdc2 levels. Of significance, p53 maintenance of G₂ arrestwas p21 and pRB dependent. Induction of p53 after cell stressresulted in a marked elevation of p21, conversion of pRB to thehypophosphorylated, active form, and increased pRB-E2F complexformation. The abrogation of pRB activity by E7 in the RKO cellsresulted in a premature G₂ exit in response to genotoxic stressand subsequent endoreduplication. Thus, our study not only providesinsight into how p53 sustains G₂ arrest after stress, it alsoshows that pRB loss can uncouple S phase and mitosis after genotoxicstress in tumorcells.

Agarwal et al. first provided evidence that p53 could mediate a G₂ growth arrest (1). The observed p53-mediated G₂ arrestin the HIp53 cells, in the absence of genotoxic stress, is consistentwith the results of this previous study. Our findings supportprevious studies demonstrating that Cdc2 is down-regulated ina p53-dependent manner after IR (3), cyclin B1 and Cdc2 levelsdecrease after ectopic p53 expression (25), and p53 expressioninhibits cyclin B1 and Cdc2 transcription (53). In agreementwith the study of Bunz et al. (5), we show that HCT116 p53^/ and HCT116 p21^/ cells are unable to maintain a G₂ arrest after exposure of cellsto IR. Our results support and provide insight into previous findingsthat pRB overexpression mediates G₂ growth arrest independentlyof p53 (26) and that hypophosphorylation of pRB occurs duringstress-induced G₂ arrest (43, 62). Further, Park et al. showthat constitutive activation of cyclin B1-Cdc2 overrides p53-mediatedG₂ arrest (37).

This study shows that similar molecular mechanisms are involved in p53 regulation of G₁ and G₂ checkpoints. The comparablemechanisms are exemplified by the results obtained after treatmentof HIp53 cells with a dose range of genotoxic agents. Exposureof HIp53 cells to lower doses of either IR or ADR, followed byp53 expression, led to a predominant G₁ cell cycle arrest, whereashigher doses of the agents caused an accumulation of cells atG₂. Analyses of cyclin B1 and Cdc2 proteins showed that a reductionin levels occurred regardless of whether a G₁ or a G₂ arrest wasinitiated if p53 was present; however, the kinetics of cyclinB1 and Cdc2 protein reduction varied and appeared to correlatewith the phase of cell cycle arrest. Exposure of cells to dosesof genotoxic agent that resulted in a predominant accumulationof cells in the G₁ phase of the cell cycle resulted in a morerapid decrease in cyclin B1 and Cdc2 protein levels compared tolevels seen after doses that resulted in a more pronounced G₂arrest. The difference in the kinetics of cyclin B1 and Cdc2 proteinloss can be explained by cell cycle-dependent gene expression.Cells in G₁ have not activated the transcription of genes thatencode G₂-phase-specific proteins, and thus cyclin B1 and Cdc2proteins are absent. In contrast, cells in G₂ have elevated levelsof cyclin B1 and Cdc2 protein. In the presence of hypophosphorylatedpRB, transcription of cyclin B1 and Cdc2 is inhibited regardlessof cell cycle phase; however, the time required for cyclin B1and Cdc2 protein degradation in a culture of cells that is predominantlyin G₂ would account for the apparent difference in kinetics ofprotein loss. These data are consistent with those of a recentstudy by de Toledo et al. which showed that down-regulation ofE2F-responsive genes, including those for Cdc2, cyclin A, cyclinB1, thymidine kinase, and topoisomerase II, occur in a p53-dependentmanner after treatment of cells with IR (10). Also, our resultsdepicting the integral role of pRB in p53-mediated maintenanceof the G₂ checkpoint response are consistent with those of a previousstudy by Hickman et al. showing that HPV E7 abrogates p53-inducedgrowth arrest and inhibition of Cdk activities (21).

An obvious question from the results presented is does the E2F family of transcription factors play a direct role in regulationof the cyclin B1 promoter? The promoters of Cdc2 and cyclin Ahave been shown to be regulated by E2F transcription factors directly(8, 9). Previous studies have demonstrated that cyclin B1expression is dependent on the kinase activity of cyclin A-Cdk2(35) and that deregulated expression of Cdk2 abrogates IR-inducedG₂ arrest (56). One possibility is that E2F regulates cyclinB1 transcription indirectly by affecting the expression of cyclinA. Alternatively, E2F transcription factors may regulate cyclinB1 transcription through direct promoter binding. In our preliminaryanalyses of the cyclin B1 promoter, we have located a putativeE2F binding element proximal to the transcriptional start site(P. M. Flatt and J. A. Pietenpol, unpublisheddata).

Several cell model systems were used in this study to show that both the ectopic expression of p53 and the activation of endogenousp53 were sufficient to sustain a G₂ arrest after stress. Our combinedresults are in contrast with the report of Passalaris et al. indicatingthat p53 does not affect the duration of G₂ arrest in responseto DNA damage (39). In the previous study, a decrease in cyclinB1 and Cdc2 protein levels in ADR-treated normal fibroblasts wasobserved; however, the change in protein levels did not affectthe length of G₂ arrest (39). Normal human fibroblasts wereused as a model system in the previous study, whereas all of thecell types used in our study were of epithelial tumor origin.We have previously shown that primary cultures of normal humankeratinocytes (epithelial) and fibroblasts (mesenchymal) havemarked differences in cell cycle checkpoint response, durationof growth arrest, and cell fate after exposure to genotoxic agents(13). Thus, the contribution of p53 at the G₂ checkpoint maybe cell type specific. In addition, Passalaris et al. used low-passage-numbercultures of normal fibroblasts for their study and noted thatincreased passage number resulted in the inability of E6-containingcells to maintain a G₂ arrest compared with fibroblasts that retainedan intact p53 signaling pathway (39). In fact, Kaufmann et al.demonstrated that E6 expression in normal human fibroblasts correlatedwith inactivation of the G₂ checkpoint and acquisition of chromosomalabnormalities (28).

A different mechanism by which p53 regulates the duration of the G₂ checkpoint is thought to be dependent on the transactivationof another p53 downstream target gene, 14-3-3 $sigma$ (20). Similarto the results with HCT116 p53^/ and HCT116 p21^/ cells, HCT116 cells null for 14-3-3 $sigma$ prematurely exit G₂ andundergo mitotic catastrophe after genotoxic stress (7). Thep53-dependent transactivation of the 14-3-3 $sigma$ gene product hasrecently been shown to play an integral role in the cytoplasmiclocalization of the cyclin B1-Cdc2 complex after genotoxic stress(7). 14-3-3 $sigma$ can form a complex with Cdc2 and wee1, and thecomplex of proteins can be identified in the cytoplasms of cellsduring G₂ arrest (7). However, as stated above, the contributionof p53 to the G₂ checkpoint response may be cell type specificsince 14-3-3 $sigma$ has not been detected in rapidly growing or irradiatedhuman diploid fibroblasts (20). Thus, inhibition of cyclin B1-Cdc2activity in response to cellular stress involves redundant biochemicalpathways that work in concert to regulate phosphorylation, subcellularlocalization, activity, and expression of cyclin B1 and Cdc2 proteins.The interplay of multiple pathways is likely required to achievethe maximal activation and maintenance of G₂ cell cycle arrestin response to cellular stress in different celltypes.

A hallmark of human tumors is deficiency of checkpoint function. Several preclinical studies have correlated loss of specificcell cycle regulatory gene products with enhanced vulnerabilityto anticancer agents (6, 19, 51, 55). There is growingevidence that ablation of G₂ arrest in tumor cell lines alterssensitivity to several anticancer agents (4, 42, 44, 45,58, 61). As we expand our understanding of how cell cycleregulatory pathways interplay to constitute a checkpoint, ourability to design rational therapies that exploit the moleculardefects in tumor cells willincrease.

	ACKNOWLEDGMENTS

Caroline D. Scatena and Luo Jia Tang contributed equally to thiswork.

We thank K. Cho for the RKO-NEO and RKO-E7 cells lines, B. Vogelstein for the isogenic set of HCT116 cells, J. Lee for thecyclin B1 promoter-CAT construct, the staff of the S. Hiebertlaboratory for assistance with the EMSA, and E. Nishida and H.Piwnica-Worms for cyclin B1 and Cdc2 cDNAs, respectively. We thankthe members of the Pietenpol laboratory for critical reading ofthemanuscript.

This work was supported by a Burroughs Wellcome New Investigator in Toxicology award (J.A.P.), NIH grant CA70856 (J.A.P.),NIEHS institutional training grant ES07028 (C.D.S.), NIH grantCA68485 (core services), and NIEHS grants ES07028 and ES00267(coreservices).

	FOOTNOTES

^* Corresponding author. Mailing address: Vanderbilt University School of Medicine, Department of Biochemistry, 652 Medical ResearchBuilding II, Nashville, TN 37232-6305. Phone: (615) 936-1512.Fax: (615) 936-2294. E-mail: pietenpol{at}toxicology.mc.vanderbilt.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Agarwal, M. L., A. Agarwal, W. R. Taylor, and G. R. Stark. 1995. p53 controls both the G₂/M and the G₁ cell cycle checkpoints and mediates reversible growth arrest in human fibroblasts. Proc. Natl. Acad. Sci. USA 92:8493-8497[Abstract/Free Full Text].

2. Agarwal, M. L., W. R. Taylor, M. V. Chernov, O. B. Chernova, and G. R. Stark. 1999. The p53 network. J. Biol. Chem. 273:1-4[Free Full Text].

3. Azzam, E. I., S. M. De Toledo, M. J. Pykett, H. Nagasawa, and J. B. Little. 1997. CDC2 is down-regulated by ionizing radiation in a p53-dependent manner. Cell Growth Differ. 8:1161-1169[Abstract].

4. Blume, E. 1995. Researchers gain footholds in the cell cycle. J. Natl. Cancer Inst. 87:1504-1505[Free Full Text].

5. Bunz, F., A. Dutriaux, C. Lengauer, T. Waldman, S. Zhou, J. P. Brown, J. M. Sedivy, K. W. Kinzler, and B. Vogelstein. 1998. Requirement for p53 and p21 to sustain G₂ arrest after DNA damage. Science 282:1497-1501[Abstract/Free Full Text].

6. Bunz, F., P. M. Hwang, C. Torrance, T. Waldman, Y. Zhang, L. Dillehay, J. Williams, C. Lengauer, K. W. Kinzler, and B. Vogelstein. 1999. Disruption of p53 in human cancer cells alters the responses to therapeutic agents. J. Clin. Investig. 104:263-269[Medline].

7. Chan, T. A., H. Hermeking, C. Lengauer, K. W. Kinzler, and B. Vogelstein. 1999. 14-3-3 sigma is required to prevent mitotic catastrophe after DNA damage. Nature 401:616-620[CrossRef][Medline].

8. Dalton, S. 1992. Cell cycle regulation of the human cdc2 gene. EMBO J. 11:1797-1804[Medline].

9. DeGregori, J., T. Kowalik, and J. R. Nevins. 1999. Cellular targets for activation by the E2F1 transcription factor include DNA synthesis- and G₁/S-regulatory genes. Mol. Cell. Biol. 15:5846-5847.

10. de Toledo, S., E. Azzam, P. Keng, S. Laffrenier, and J. Little. 1998. Regulation by ionizing radiation of CDC2, cyclin A, cyclin B, thymidine kinase, topoisomerase IIa, and RAD51 expression in normal human diploid fibroblasts is dependent on p53/p21. Cell Growth Differ. 9:887-896[Abstract].

11. Demers, G. W., S. A. Foster, C. L. Halbert, and D. A. Galloway. 1994. Growth arrest by induction of p53 in DNA damaged keratinocytes is bypassed by human papillomavirus 16 E7. Proc. Natl. Acad. Sci. USA 91:4382-4386[Abstract/Free Full Text].

12. El-Deiry, W. S., S. E. Kern, J. A. Pietenpol, K. W. Kinzler, and B. Vogelstein. 1992. Definition of a consensus binding site for p53. Nat. Genet. 1:45-49[CrossRef][Medline].

13. Flatt, P. M., J. O. Price, A. Shaw, and J. A. Pietenpol. 1998. Differential cell cycle checkpoint response in normal human keratinocytes and fibroblasts. Cell Growth Differ. 9:535-543[Abstract].

14. Furukawa, Y., Y. Terui, K. Sakoe, M. Ohta, and M. Saito. 1994. The role of cellular transcription factor E2F in the regulation of cdc2 mRNA expression and cell cycle control of human hematopoietic cells. J. Biol. Chem. 269:26249-26258[Abstract/Free Full Text].

15. Graeber, T. G., J. F. Peterson, M. Tsai, K. Monica, A. J. Fornance, Jr., and A. J. Giaccia. 1994. Hypoxia induces accumulation of p53 protein, but activation of a G₁-phase checkpoint by low-oxygen conditions is independent of p53 status. Mol. Cell. Biol. 14:6264-6277[Abstract/Free Full Text].

16. Harper, J. W., G. R. Adami, N. Wei, K. Keyomarsi, and S. J. Elledge. 1993. The p21 Cdk-interacting protein Cip1 is a potent inhibitor of G1 cyclin-dependent kinases. Cell 75:805-816[CrossRef][Medline].

17. Hartwell, L. H., and T. A. Weinert. 1989. Checkpoints: controls that ensure the order of cell cycle events. Science 246:629-634[Abstract/Free Full Text].

18. Haupt, Y., R. Maya, A. Kazaz, and M. Oren. 1997. Mdm2 promotes the rapid degradation of p53. Nature 387:296-299[CrossRef][Medline].

19. Hawkins, D. S., G. W. Demers, and D. A. Galloway. 1996. Inactivation of p53 enhances sensitivity to multiple chemotherapeutic agents. Cancer Res. 56:892-898[Abstract/Free Full Text].

20. Hermeking, H., C. Lengauer, K. Polyak, T.-C. He, L. Zhang, S. Thiagalingam, K. W. Kinzler, and B. Vogelstein. 1998. 14-3-3 $sigma$ is a p53-regulated inhibitor of G2/M progression. Mol. Cell 1:3-11.

21. Hickman, E. S., S. Bates, and K. H. Vousden. 1997. Perturbation of the p53 response by human papillomavirus type 16 E7. J. Virol. 71:3710-3718[Abstract].

22. Hiebert, S. W., S. Chellappan, J. M. Horowitz, and J. R. Nevins. 1992. The interaction of RB with E2F coincides with inhibition of the transcriptional activity of E2F. Genes Dev. 6:177-185[Abstract/Free Full Text].

23. Hiebert, S. W., G. Packham, D. K. Strom, R. Haffner, M. Oren, G. Zambetti, and J. L. Cleveland. 1995. E2F-1:DP-1 induces p53 and overrides survival factors to trigger apoptosis. Mol. Cell. Biol. 15:6864-6874[Abstract].

24. Hussain, S. P., and C. C. Harris. 1999. p53 mutation spectrum and load: the generation of hypotheses linking the exposure of endogenous or exogenous carcinogens to human cancer. Mutat. Res. 428:23-32[Medline].

25. Innocente, S. A., J. L. A. Abrahamson, J. P. Cogswell, and J. M. Lee. 1999. p53 regulates a G₂ checkpoint through cyclin B1. Proc. Natl. Acad. Sci. USA 96:2147-2152[Abstract/Free Full Text].

26. Karantza, V., A. Maroo, D. Fay, and J. M. Sedivy. 1993. Overproduction of Rb protein after the G₁/S boundary causes G₂ arrest. Mol. Cell. Biol. 13:6640-6652[Abstract/Free Full Text].

27. Kastan, M. B., O. Onyekwere, D. Sidransky, B. Vogelstein, and R. W. Craig. 1991. Participation of p53 protein in the cellular response to DNA damage. Cancer Res. 51:6304-6311[Medline].

28. Kaufmann, W. K., J. L. Schwartz, J. C. Hurt, L. L. Byrd, D. A. Galloway, E. Levedakou, and R. S. Paules. 1997. Inactivation of G₂ checkpoint function and chromosomal destabilization are linked in human fibroblasts expressing human papillomavirus type 16 E6. Cell Growth Differ. 8:1105-1114[Abstract].

29. Kern, S. E., J. A. Pietenpol, S. Thiagalingam, A. Seymour, K. W. Kinzler, and B. Vogelstein. 1992. Oncogenic forms of p53 inhibit p53-regulated gene expression. Science 256:827-830[Abstract/Free Full Text].

30. Kubbutat, M. H. G., S. N. Jones, and K. H. Vousden. 1997. Regulation of p53 stability by Mdm2. Nature 387:299-303[CrossRef][Medline].

31. Li, C. Y., H. Nagasawa, W. K. Dahlberg, and J. B. Little. 1995. Diminished capacity for p53 in mediating a radiation-induced G₁ arrest in established human tumor cell lines. Oncogene 11:1885-1892[Medline].

32. Lowe, S. W., and H. E. Ruley. 1993. Stabilization of the p53 tumor suppressor is induced by adenovirus 5 E1A and accompanies apoptosis. Genes Dev. 7:535-545[Abstract/Free Full Text].

33. Lowe, S. W., E. M. Schmitt, S. W. Smith, B. A. Osborne, and T. Jacks. 1993. p53 is required for radiation-induced apoptosis in mouse thymocytes. Nature 362:847-849[CrossRef][Medline].

34. Morgan, D. O. 1995. Principles of CDK regulation. Nature 374:131-134[CrossRef][Medline].

35. Moro, A., K. Zerfass, S. Joswig, and P. Jansen-Duerr. 1997. Effect of cyclins and Cdks on the cyclin B1 promoter activation. Biochem. Mol. Biol. Int. 41:919-924[Medline].

36. Mueller, P. R., T. R. Coleman, A. Kumagai, and A. Dunphy. 1995. Myt1: a membrane-associated inhibitory kinase that phosphorylates cdc2 on both threonine-14 and tyrosine-15. Science 270:86-93[Abstract/Free Full Text].

37. Park, M., H. D. Chae, J. Yun, M. Jung, Y. S. Kim, S. H. Kim, M. H. Han, and D. Y. Shin. 2000. Constitutive activation of cyclin B1-associated cdc2 kinase overrides p53-mediated G₂-M arrest. Cancer Res. 60:542-545[Abstract/Free Full Text].

38. Parker, L. L., and H. Piwnica-Worms. 1992. Inactivation of p34^cdc2-cyclin B complex by the human WEE1 tyrosine kinase. Science 257:1955-1957[Abstract/Free Full Text].

39. Passalaris, T. M., J. A. Benanti, L. Gewin, T. Kiyono, and D. A. Galloway. 1999. The G₂ checkpoint is maintained by redundant pathways. Mo

1.	Agarwal, M. L., A. Agarwal, W. R. Taylor, and G. R. Stark. 1995. p53 controls both the G₂/M and the G₁ cell cycle checkpoints and mediates reversible growth arrest in human fibroblasts. Proc. Natl. Acad. Sci. USA 92:8493-8497[Abstract/Free Full Text].
2.	Agarwal, M. L., W. R. Taylor, M. V. Chernov, O. B. Chernova, and G. R. Stark. 1999. The p53 network. J. Biol. Chem. 273:1-4[Free Full Text].
3.	Azzam, E. I., S. M. De Toledo, M. J. Pykett, H. Nagasawa, and J. B. Little. 1997. CDC2 is down-regulated by ionizing radiation in a p53-dependent manner. Cell Growth Differ. 8:1161-1169[Abstract].
4.	Blume, E. 1995. Researchers gain footholds in the cell cycle. J. Natl. Cancer Inst. 87:1504-1505[Free Full Text].
5.	Bunz, F., A. Dutriaux, C. Lengauer, T. Waldman, S. Zhou, J. P. Brown, J. M. Sedivy, K. W. Kinzler, and B. Vogelstein. 1998. Requirement for p53 and p21 to sustain G₂ arrest after DNA damage. Science 282:1497-1501[Abstract/Free Full Text].
6.	Bunz, F., P. M. Hwang, C. Torrance, T. Waldman, Y. Zhang, L. Dillehay, J. Williams, C. Lengauer, K. W. Kinzler, and B. Vogelstein. 1999. Disruption of p53 in human cancer cells alters the responses to therapeutic agents. J. Clin. Investig. 104:263-269[Medline].
7.	Chan, T. A., H. Hermeking, C. Lengauer, K. W. Kinzler, and B. Vogelstein. 1999. 14-3-3 sigma is required to prevent mitotic catastrophe after DNA damage. Nature 401:616-620[CrossRef][Medline].
8.	Dalton, S. 1992. Cell cycle regulation of the human cdc2 gene. EMBO J. 11:1797-1804[Medline].
9.	DeGregori, J., T. Kowalik, and J. R. Nevins. 1999. Cellular targets for activation by the E2F1 transcription factor include DNA synthesis- and G₁/S-regulatory genes. Mol. Cell. Biol. 15:5846-5847.
10.	de Toledo, S., E. Azzam, P. Keng, S. Laffrenier, and J. Little. 1998. Regulation by ionizing radiation of CDC2, cyclin A, cyclin B, thymidine kinase, topoisomerase IIa, and RAD51 expression in normal human diploid fibroblasts is dependent on p53/p21. Cell Growth Differ. 9:887-896[Abstract].
11.	Demers, G. W., S. A. Foster, C. L. Halbert, and D. A. Galloway. 1994. Growth arrest by induction of p53 in DNA damaged keratinocytes is bypassed by human papillomavirus 16 E7. Proc. Natl. Acad. Sci. USA 91:4382-4386[Abstract/Free Full Text].
12.	El-Deiry, W. S., S. E. Kern, J. A. Pietenpol, K. W. Kinzler, and B. Vogelstein. 1992. Definition of a consensus binding site for p53. Nat. Genet. 1:45-49[CrossRef][Medline].
13.	Flatt, P. M., J. O. Price, A. Shaw, and J. A. Pietenpol. 1998. Differential cell cycle checkpoint response in normal human keratinocytes and fibroblasts. Cell Growth Differ. 9:535-543[Abstract].
14.	Furukawa, Y., Y. Terui, K. Sakoe, M. Ohta, and M. Saito. 1994. The role of cellular transcription factor E2F in the regulation of cdc2 mRNA expression and cell cycle control of human hematopoietic cells. J. Biol. Chem. 269:26249-26258[Abstract/Free Full Text].
15.	Graeber, T. G., J. F. Peterson, M. Tsai, K. Monica, A. J. Fornance, Jr., and A. J. Giaccia. 1994. Hypoxia induces accumulation of p53 protein, but activation of a G₁-phase checkpoint by low-oxygen conditions is independent of p53 status. Mol. Cell. Biol. 14:6264-6277[Abstract/Free Full Text].
16.	Harper, J. W., G. R. Adami, N. Wei, K. Keyomarsi, and S. J. Elledge. 1993. The p21 Cdk-interacting protein Cip1 is a potent inhibitor of G1 cyclin-dependent kinases. Cell 75:805-816[CrossRef][Medline].
17.	Hartwell, L. H., and T. A. Weinert. 1989. Checkpoints: controls that ensure the order of cell cycle events. Science 246:629-634[Abstract/Free Full Text].
18.	Haupt, Y., R. Maya, A. Kazaz, and M. Oren. 1997. Mdm2 promotes the rapid degradation of p53. Nature 387:296-299[CrossRef][Medline].
19.	Hawkins, D. S., G. W. Demers, and D. A. Galloway. 1996. Inactivation of p53 enhances sensitivity to multiple chemotherapeutic agents. Cancer Res. 56:892-898[Abstract/Free Full Text].
20.	Hermeking, H., C. Lengauer, K. Polyak, T.-C. He, L. Zhang, S. Thiagalingam, K. W. Kinzler, and B. Vogelstein. 1998. 14-3-3 $sigma$ is a p53-regulated inhibitor of G2/M progression. Mol. Cell 1:3-11.
21.	Hickman, E. S., S. Bates, and K. H. Vousden. 1997. Perturbation of the p53 response by human papillomavirus type 16 E7. J. Virol. 71:3710-3718[Abstract].
22.	Hiebert, S. W., S. Chellappan, J. M. Horowitz, and J. R. Nevins. 1992. The interaction of RB with E2F coincides with inhibition of the transcriptional activity of E2F. Genes Dev. 6:177-185[Abstract/Free Full Text].
23.	Hiebert, S. W., G. Packham, D. K. Strom, R. Haffner, M. Oren, G. Zambetti, and J. L. Cleveland. 1995. E2F-1:DP-1 induces p53 and overrides survival factors to trigger apoptosis. Mol. Cell. Biol. 15:6864-6874[Abstract].
24.	Hussain, S. P., and C. C. Harris. 1999. p53 mutation spectrum and load: the generation of hypotheses linking the exposure of endogenous or exogenous carcinogens to human cancer. Mutat. Res. 428:23-32[Medline].
25.	Innocente, S. A., J. L. A. Abrahamson, J. P. Cogswell, and J. M. Lee. 1999. p53 regulates a G₂ checkpoint through cyclin B1. Proc. Natl. Acad. Sci. USA 96:2147-2152[Abstract/Free Full Text].
26.	Karantza, V., A. Maroo, D. Fay, and J. M. Sedivy. 1993. Overproduction of Rb protein after the G₁/S boundary causes G₂ arrest. Mol. Cell. Biol. 13:6640-6652[Abstract/Free Full Text].
27.	Kastan, M. B., O. Onyekwere, D. Sidransky, B. Vogelstein, and R. W. Craig. 1991. Participation of p53 protein in the cellular response to DNA damage. Cancer Res. 51:6304-6311[Medline].
28.	Kaufmann, W. K., J. L. Schwartz, J. C. Hurt, L. L. Byrd, D. A. Galloway, E. Levedakou, and R. S. Paules. 1997. Inactivation of G₂ checkpoint function and chromosomal destabilization are linked in human fibroblasts expressing human papillomavirus type 16 E6. Cell Growth Differ. 8:1105-1114[Abstract].
29.	Kern, S. E., J. A. Pietenpol, S. Thiagalingam, A. Seymour, K. W. Kinzler, and B. Vogelstein. 1992. Oncogenic forms of p53 inhibit p53-regulated gene expression. Science 256:827-830[Abstract/Free Full Text].
30.	Kubbutat, M. H. G., S. N. Jones, and K. H. Vousden. 1997. Regulation of p53 stability by Mdm2. Nature 387:299-303[CrossRef][Medline].
31.	Li, C. Y., H. Nagasawa, W. K. Dahlberg, and J. B. Little. 1995. Diminished capacity for p53 in mediating a radiation-induced G₁ arrest in established human tumor cell lines. Oncogene 11:1885-1892[Medline].
32.	Lowe, S. W., and H. E. Ruley. 1993. Stabilization of the p53 tumor suppressor is induced by adenovirus 5 E1A and accompanies apoptosis. Genes Dev. 7:535-545[Abstract/Free Full Text].
33.	Lowe, S. W., E. M. Schmitt, S. W. Smith, B. A. Osborne, and T. Jacks. 1993. p53 is required for radiation-induced apoptosis in mouse thymocytes. Nature 362:847-849[CrossRef][Medline].
34.	Morgan, D. O. 1995. Principles of CDK regulation. Nature 374:131-134[CrossRef][Medline].
35.	Moro, A., K. Zerfass, S. Joswig, and P. Jansen-Duerr. 1997. Effect of cyclins and Cdks on the cyclin B1 promoter activation. Biochem. Mol. Biol. Int. 41:919-924[Medline].
36.	Mueller, P. R., T. R. Coleman, A. Kumagai, and A. Dunphy. 1995. Myt1: a membrane-associated inhibitory kinase that phosphorylates cdc2 on both threonine-14 and tyrosine-15. Science 270:86-93[Abstract/Free Full Text].
37.	Park, M., H. D. Chae, J. Yun, M. Jung, Y. S. Kim, S. H. Kim, M. H. Han, and D. Y. Shin. 2000. Constitutive activation of cyclin B1-associated cdc2 kinase overrides p53-mediated G₂-M arrest. Cancer Res. 60:542-545[Abstract/Free Full Text].
38.	Parker, L. L., and H. Piwnica-Worms. 1992. Inactivation of p34^cdc2-cyclin B complex by the human WEE1 tyrosine kinase. Science 257:1955-1957[Abstract/Free Full Text].
39.	Passalaris, T. M., J. A. Benanti, L. Gewin, T. Kiyono, and D. A. Galloway. 1999. The G₂ checkpoint is maintained by redundant pathways. Mo